Human phospholipase a2 epsilon

ABSTRACT

A novel function phospholipase A 2 , referred to herein as calcium-independent phospholipase A 2ε  (iPLA 2ε ) having SEQ ID NO: 1 and SEQ ID NO: 2, and nucleic acid sequences (SEQ ID NO: 3 and SEQ ID NO: 4) encoding and expressing iPLA 2 ε is disclosed. This novel enzyme has been isolated and characterized and is involved in the catalysis and hydrolysis of lipids cycling in a living cell biosystem. In an embodiment, the iPLA 2 ε polypeptide is encoded and expressed by an isolated nucleic acid molecule comprising a set of iPLA 2 ε polynucleotides. In one aspect, an isolated and characterized gene comprises a polynucleotide having a sequence shown in SEQ ID NO: 3 and SEQ ID NO: 4.

CROSS REFERENCE TO RELATED APPLICATIONS

This application is a divisional application of U.S. application Ser. No. 11/010,558 filed Dec. 13, 2004, which claims the benefit of U.S. provisional patent application 60/528,951 filed Dec. 11, 2003. The contents of these applications are incorporated herein by reference in their entireties.

STATEMENT REGARDING FEDERALLY SPONSORED RESEARCH AND DEVELOPMENT

This research was supported jointly by grants from the National Institutes of Health grants 5P01HL57278-06A1 and 5R01HL41250-10. The government has certain rights in the invention.

FIELD OF THE INVENTION

This discovery relates to phospholipases, lipases and transacylases and to a method for using them. More particularly this discovery relates to a method for screening drugs.

BACKGROUND OF THE INVENTION

Unfortunately in many industrialized countries, the incidence of human obesity is dramatically increasing. Moreover, human obesity is a common and costly nutritional problem in the United States in addition to being a devastating health problem. Obesity is characterized clinically by the accumulation of fat tissue (at times this is referred to as body fat content).

In humans, obesity is usually defined as a body fat content greater than about 25% of the total weight for males, or greater than about 30% of the total weight for females. However obesity exists outside those numbers too. Regardless of the cause of or extent of obesity, obesity is an ever present problem for Americans. But a fat content greater than about 18% for males and greater than about 22% for females can have untold consequences secondary to several mechanisms and disorders of metabolic function. For example, obesity can have a significant adverse impact on health care costs and provoke a higher risk of numerous illnesses, including heart attacks, strokes and diabetes.

In the case of diabetes, patients can lose limbs, eyesight and kidneys and hearts can fail so the potential results can be catastrophic and deadly.

Without being bound by theory, it is believed that obesity in humans results from an abnormal increase in white adipose tissue mass that occurs due to an increased number of adipocytes (hyperplasia) or from increased lipid mass accumulating in existing adipocytes. Obesity and the associated type two metabolic syndrome along with its clinical sequelae are among the major and the most rapidly increasing (epidemic) medical problems in America. However, to date, a lack of suitable adipocyte specific protein targets has unfortunately hampered progress in the development of effective therapeutic agents to combat the clinical sequelae of obesity.

Despite existing knowledge of the critical role of phospholipases in adipocyte signaling, enhanced clinical methodology and research tool and methods are highly needed for new obesity drugs and new methods for identifying useful drugs to treat obesity and over-weightness. It is highly desired to have knowledge and technology based on the specific types of phospholipases and lipases present in the adipocyte, or their mechanisms of regulation, and determine their natural substrates and roles in anabolic lipid metabolism, catabolic lipid metabolism or both (e.g. triglyceride cycling).

BRIEF DESCRIPTION OF THE INVENTION

This invention relates to phospholipases, lipases and transacylases and more particularly to human calcium independent phospholipase A₂ε, hereinafter referred to as and denoted (iPLA₂ε, also denoted as iPLA₂ epsilon), to nucleic acids expressing iPLA₂ε, to the use of iPLA₂ε as a pharmacological target in screening and development of potentially useful anti-obesity drugs and drugs for other sequelae of the metabolic syndrome including at least one of atherosclerosis, diabetes, cancer and hypertension and to an animal model useful for such screening.

In an aspect, the invention provides for the first time an isolated novel, purified, recovered, functional and characterized human phospholipase A₂, referred to herein as calcium-independent phospholipases A₂ε (iPLA₂ε) having SEQ ID NO: (See FIG. 3A) and SEQ ID NO: 2 (See FIG. 3B), and nucleic acid sequences (SEQ ID NO: 3) and (SEQ ID NO: 4) SNP's thereof encoding and expressing iPLA₂ε activity (See FIGS. 3A and 3B). For the first time herein, this novel enzyme(s) has been isolated, recovered, purified and characterized. iPLA₂ε is involved in the catalysis, synthesis and hydrolysis of lipids in a living mammalian cell. Moreover, through the process of transesterification the inventors have discovered that this enzyme iPLA₂ε can catalyze the net anabolic synthesis of triglycerides through a variety of metabolic precursor's (e.g. monoacylglycerol, diacylglycerol and acyl CoA).

In one aspect, the invention is directed to an isolated, recovered, and characterized functional nucleic acid molecule comprising a set of iPLA₂ε polynucleotides. In a further aspect of the iPLA₂ε polynucleotides encode and express an iPLA₂ε polypeptide.

In one aspect, an isolated, recovered, functional, characterized human gene comprises an isolated and characterized polynucleotide having a sequence shown in SEQ ID NO: 3 and SEQ ID NO: 4. (See FIGS. 3A and 3B).

In an aspect, an isolated, recovered, functional, characterized human protein comprises a polypeptide having a sequence shown in SEQ ID NO: 1 and SEQ ID NO: 2 (See FIGS. 3A and 3B).

In an aspect, this discovery comprises a method to successfully measure lipase activity in fat cells and its inhibition by BEL. This discovery provides a useful screening method and research tool to identify useful drugs which can be effectively administered to patients afflicted with diabetes, overweight and obesity.

In an aspect, a method of effectively treating a living mammal to reduce obesity, comprises administering an effective amount iPLA₂ε inhibitor thereto or an agent which changes the lipase to transacylase ratio.

In an aspect, a genetically engineered isolated, functional, characterized functional expression vector comprises a functional gene or part of the sequence of a human gene comprising a polynucleotide having a sequence shown in SEQ ID NO: 3 or SEQ ID NO: 4 (FIGS. 3A and 3B). In an aspect, the gene encodes a protein comprising a polypeptide having a sequence shown in SEQ ID NO: 1 or SEQ ID NO: 2 (FIGS. 3A and 3B). In an aspect, the gene is operatively linked to a capable viable promoter element.

In another aspect, a method of medically treating a mammal comprises administering an anti-obesity (drug or pharmaceutical) in therapeutically effective amounts as an inhibitor to the living mammal.

In another aspect, a method of effectively medically treating at a clinical level a living mammal and comprises administering a therapeutically effective amount of a compound (drug or pharmaceutical) which inhibits iPLA₂ε expression to the mammal or result in a different isoform expression or different enzymatic activity or post-translational modification.

In another aspect, a method of treating obesity, at a clinical situation or level comprising administering an agent which changes the transacylase to lipase ratio in a metabolic setting. In an aspect, the metabolic setting is a living animal or an adequately representative animal model. In an aspect the agent compresses a compound.

In an aspect, a pharmaceutical composition is provided comprising a compound which effectively inhibits or counteracts iPLA₂ε expression, activity, hydrolysis or transesterification activity or transesterification in a living mammal such as a human.

In an aspect, a pharmaceutical kit comprises a container housing a compound which effectively inhibits at least one of iPLA₂ε expression, activity or transesterification.

In another embodiment, the present invention is directed to a method of modulating fatty acid utilization in a living patient. In an aspect, the patient is a living human patient. In this aspect, the method comprises intentionally and selectively increasing or decreasing iPLA₂ε activity in the patient. Patients in need of such treatment include those patients suffering from one of diabetes and/or obesity. Preferably, this method comprises administering to the patient a substance (compound) in an effective amount which blocks or inhibits expression of iPLA₂ε mass or activity.

In an aspect a method of identifying an agent which changes the ratio of transacylase to lipase in a living mammal by administering a compound to a mammal and determining if the transacylase to lipase ratio was changed by lipid analysis and if the ratio was changed then determining that the drug is an anti-obesity drug.

In an aspect, the invention comprises a method for ameliorating at least one symptom of a symptomatology comprising obesity and the clinical manifestations of the type 2 metabolic syndrome in a living human which comprises treating a human cell expressing iPLA₂ε in a pharmacologically effective manner with a pharmacologically effective amount of an iPLA₂ε expression or enzymatic inhibitor. In an aspect the human body is treated by treating the cells thereof.

A method of treating at least one of an overweight and obese disorders, the method comprises administering to a subject (in need of such treatment) a therapeutically effective amount of composition comprising an inhibitor of human or murine iPLA₂ε (adiponutrin).

In an aspect, a method of identifying an anti-obesity drug which comprises administering a drug to an animal and determining if there has been any change in iPLA₂ε expression, activity, hydrolysis or transesterification activity or futile cycles and if so determining that the drug is an anti-obesity drug.

In an aspect a method of practicing medicine comprises administering a therapeutic amount of a drug to a living patient at risk for obesity or being obese, the drug being an inhibitor of human adiponutrin (iPLA₂ε).

In an aspect a method of providing therapy to a patient in need thereof which comprises administering a drug to a patient at risk for obesity, the drug being an inhibitor of the expression of human adiponutrin (iPLA₂ε).

In an aspect a method for treating a diabetic comprises administering a drug to a patient in a pharmacologically effective amount to modulate iPLA₂ε expression whereby the insulin requirement of the patient is decreased. In an aspect the patient presents clinically determined symptoms of diabetes.

In an aspect a method of treating diabetes comprises administering a drug in an effective amount to modulate iPLA₂ε expression whereby the insulin requirement of the patient is decreased.

In an aspect an antibody which recognizes human iPLA₂ε comprises a peptide corresponding to residues 295-310 of human iPLA₂ε (CRLEGDELLDHLRLSIL) (SEQ ID NO:9).

In an aspect an animal model which provides at least one of a genomic target and a pharmacological target respectively comprising iPLA₂ε for reactive reception to at least one of a projectile comprising siRNA or from a pharmacological drug administered to the animal model. In an aspect, the animal model is a living tissue representative of a living animal or a sample of a living animal such as tissue. In an aspect, the pharmacological drug is a drug being evaluated.

In an aspect, the present discovery also encompasses genetically engineered cells capable of identifying substances which modulate iPLA₂ε expression in a living biosystem cell or in a sample adequately representative thereof. In an aspect, such cells comprise a promoter operably linked to iPLA₂ε gene and a reporter gene. This reporter gene preferably encodes an enzyme capable of being detected by at least one of a suitable radiometric, fluorimetric or luminometric assay such as, for example, a reporter sequence encoding a luciferase. In an aspect, the promoter sequence is a baculovirus promoter sequence and the cells are Sf9 cells.

In an aspect, the invention comprises a method for prioritizing the therapeutic capability of a drug's putative efficacy against obesity, comprising administering drugs to a living animal system which is actively expressing iPLA₂ε, measuring any modulation of the iPLA₂ε expression by a TAG or FFA's/glycerol analysis of an effect and determining if the modulation was an increase or a decrease or no change in iPLA₂ε expression level. If the modulation is determined to be a decrease then determining that the drug was effective in inhibiting iPLA₂ε, a value is assigned to that modulation and is thereafter compared to the modulation of other drugs. In an aspect, a prioritization is set up by comprising the magnitudes of the various respective modulations and a hierarchy of drugs is established. From this, it is possible to a priority of work on the drugs is determined with a focus on their therapeutic capability.

In an aspect the iPLA₂ε can function as a signaling enzyme to control eicosanoid synergies and other lipids and messengers of signal transduction. In an aspect a method of attenuating eicosanoid synergies, lipids and messengers of signal transduction by increasing or decreasing the amount of iPLA₂ε present in a living biosystem such as a living mammal.

In an aspect, the discovery comprises a method to utilize the selective cleavage of arachidonic acid containing phospholipids mediated by iPLA₂ε to screen for inhibitors which can affect the metabolic syndrome and/or result in a change in the weight status, insulin sensitivity, or inflammatory status of the patient and organs and vessels contained therein.

The present invention also includes a method and research tool useful for identifying substances such as a compound, cell or substance or moiety which modulate iPLA₂ε expression. In an aspect, a screening method and research tool herein comprises a screening method comprising contacting a candidate substance with cells capably expressing at least a significant amount of iPLA₂ε or a fragment thereof, and measuring the expression of iPLA₂ε or a fragment thereof by the cells by an analysis of an effluent for the TAG content determining whether a substance modulated iPLA₂ε expression by measuring the expression of iPLA₂ε.

BRIEF DESCRIPTION OF THE DRAWINGS

FIG. 1 shows a schematic diagram of Adipocyte Acyl-CoA-Independent Triglyceride Cycling in a living human.

FIG. 2 shows the Calcium-Independent Phospholipase A₂ (iPLA₂) Gene Family and Sequence Alignment of iPLA₂ Nucleotide and Lipase Consensus Motifs. Members of the iPLA₂ gene family (α (SEQ ID NO: 5), β (SEQ ID NO: 6), γ (SEQ ID NO: 7), and ε (SEQ ID NO: 8)) are aligned according to their conserved nucleotide-binding motifs (open bars) and lipase consensus sites (filled bars).

FIG. 3A and FIG. 3 B show Nucleotide and Deduced Amino Acid Sequences of Our Human Adiponutrin (iPLA₂ε) and variants thereof.

FIG. 4 shows Western Analysis of the Subcellular Localization of Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10).

FIG. 5A shows Phospholipase A₂ Activity of Recombinant iPLA₂ε(His)₆.

FIG. 5B shows Phospholipase A₂ Activity of Affinity Purified Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10).

FIG. 5C shows Inhibition of Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) Phospholipase A₂ Activity by (E)-6-(bromomethylene)-3-(1-naphthalenyl)-2H-tetrahydropyran-2-one (BEL).

FIG. 6A shows Triolein Lipase Activity of Sf9 Subcellular Fractions Containing Recombinant Human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10).

FIG. 6B shows Inhibition of Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) Triolein Lipase Activity by BEL.

FIG. 6C shows Inhibition of Affinity Purified Recombinant Human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) Triolein Lipase Activity by BEL.

FIG. 7 shows TALON-Co²⁺ Affinity Chromatography of Recovered Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10).

FIG. 8 shows Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) Catalyzes Transacylation of [¹⁴C]-Mono-olein Mono-olein (donor) to Mono-olein and Diolein (acceptors) to form Triolein.

FIG. 9 shows Affinity Purified Recombinant iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) Catalyzes Transacylation of Mono-olein to Form Diolein and Triolein.

FIG. 10 shows effective and successful Inhibition of 3T3-L1 Triolein Lipase Activity by BEL.

FIG. 11 shows our Modulation of Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) Lipase/Transacylase Ratio by BEL.

FIG. 12 shows Quantitative PCR or iPLA₂ε Message in Mouse 3T3-L1 Preadipocytes and Human SW872 Liposarcoma Cells.

DETAILED DESCRIPTION OF THE DRAWINGS

FIG. 1 presents a schematic diagram of Adipocyte Acyl-CoA-Independent Triglyceride Cycling in a living human. The inventors have discovered that acyl-equivalents are stored in the adipocyte primarily in the form of triglycerides which are synthesized by iPLA₂ε (Adiponutrin), iPLA₂ε, and/or iPLA₂ε through an acyl-CoA independent transacylation mechanism which transfers fatty acyl moieties from monoacylglycerol (MAG) or diacylglycerol (DAG) acyl-donors to MAG and DAG acyl-acceptor intermediates to and from triacylglycerols (TAG) and that, alternatively, hydrolysis of a single TAG fatty acyl moiety is catalyzed by iPLA₂ε (Adiponutrin), iPLA₂ε, and/or iPLA₂ε to form DAG which can then be further degraded to MAG and glycerol by either iPLA₂ε (Adiponutrin), iPLA₂ε, iPLA₂ε and/or other intracellular lipases (e.g. hormone sensitive lipase (HSL)).

FIG. 2 shows the Calcium-Independent Phospholipase A₂ (iPLA₂) Gene Family and Sequence Alignment of iPLA₂ Nucleotide and Lipase Consensus Motifs. Members of the iPLA₂ gene family (α, β, γ, . . . and ε) are aligned according to their conserved nucleotide-binding motifs (open bars) and lipase consensus sites (filled bars). Calcium-independent phospholipase A₂ β contains eight ankyrin repeat domains (boxed horizontal bars) and a calmodulin-binding domain (CaM) near the C-terminus (boxed diagonal bars).

FIGS. 3A and 3B provide_Nucleotide and Deduced Amino Acid Sequences of Our Newly Discovery Human Adiponutrin (iPLA₂ε) and variants thereof. A. Glu434 Variant (refSNP ID=2294918 (g); Sequence ID+AK025665 (nucleotide)) B. Lys434 Variant (refSNP ID=2294918(a); Sequence ID=AL138578.2 (nucleotide): NP_(—)079501 (protein)). The depicted nucleotide coding sequences (lower case letters) of human adiponutrin (1446 bp) encode for polypeptides of 481 amino acids (upper case letters). The amino acid encoded for each adiponutrin (iPLA₂ε) allelic variant is boxed. The conserved nucleotide binding (GCGFLG) and lipase (GASAG) consensus sequences are indicated with dashed and solid lines, respectively. The catalytic serine (Ser-47) is depicted to illustrate the native (where R═H) or acylated enzyme (where R=any fatty acyl moiety).

FIG. 3A and FIG. 3B show our novel nucleic acids and our novel enzymes claimed herein as iPLA₂ε. SEQ ID#'s (for page 2 herein) are at the top of FIGS. 3A and 3B. SEQ ID NO. 1 is FIG. 3A (listed protein sequence); SEQ ID NO. 2 is FIG. 3B (listed protein sequence); SEQ ID NO. 3 is FIG. 3A (listed nucleotide sequence); and SEQ ID NO. 4 is FIG. 3B (listed nucleotide sequence) such variants are included herein as iPLA₂ε.^(˜)

FIG. 4 shows Western Analysis of the Subcellular Localization of Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10). Sf9 cells infected with either control empty-vector pFastBac (pFB) or pFB encoding human adiponutrin (iPLA₂ε) for 48 h were pelleted, washed once in ice-cold phosphate buffered saline, and resuspended in 25 mM sodium phosphate buffer, pH 7.0 containing 20% glycerol and 2 mM 2-mercaptoethanol. After lysis by sonication, cytosol (Cyto) and membrane (Memb) fractions were isolated by ultracentrifugation (100,000×g for 1 h). Proteins from the cytosol and membrane fractions were resolved by SDS-PAGE (50 μg/lane), transferred to a PVDF membrane, and probed with an antibody immunoreactive toward residues 295-310 of human adiponutrin (iPLA₂ε). Immunoreactive bands were visualized by enhanced chemiluminescence (ECL) following incubation of the blot with a protein A-horse radish peroxidase conjugate.

FIG. 5A shows Phospholipase A₂ Activity of Recombinant iPLA₂ε(His)₆. Sf9 cytosol and membrane fractions were isolated from pFB control and human adiponutrin (iPLA₂ε)-expressing cells (iPLA₂ε) as described more particularly hereafter. Subcellular fractions were incubated with 1-palmitoyl-2-[1-¹⁴C]-oleoyl-sn-glycero-3-phosphatidylcholine in the presence of 100 mM Tris-HCl, pH 7.5 containing either 10 mM CaCl₂ or 4 mM EGTA at 37° C. for 5 min. Radiolabeled product and remaining substrate were extracted into butanol, resolved by thin-layer chromatography, and quantified by scintillation spectrometry as described more particularly hereafter.

FIG. 5B shows Phospholipase A₂ Activity of Affinity Purified Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10). Affinity purified recombinant human adiponutrin (iPLA₂ε(His)₆) was incubated in 100 mM Tris-HCl, pH 7.2 containing 4 mM EGTA (200 μl final volume) for 30 min at 37° C. in the presence of 1-palmitoyl-2-[1-¹⁴C]-oleoyl-sn-glycero-3-phosphocholine (POPC), 1-palmitoyl-2-[1-¹⁴C]-linoleoyl-sn-glycero-3-phosphocholine (PLPC), or 1-palmitoyl-2-[1-¹⁴C]-arachidonyl-sn-glycerol-3-phosphocholine (PAPC) introduced by ethanolic injection. Reactions were terminated by addition of 100 μl of butanol and extraction of the radiolabeled product and remaining substrate into the butanol layer by vigorous vortexing. Samples were spotted on LK6 Silica Gel 60 Å TLC plates, overlaid with oleic acid standard, dried, and developed in petroleum ether/ethyl ether/acetic acid (70:30:1). The region of the plate corresponding to the oleic acid standard (visualized by iodine staining) was scraped into scintillation vials and quantified by liquid scintillation spectrometry.

FIG. 5C shows Inhibition of Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) Phospholipase A₂ activity by (E)-6-(bromomethylene)-3-(1-naphthalenyl)-2H-tetrahydropyran-2-one (BEL). Affinity purified human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) was pre-incubated with the indicated concentrations of (R)-BEL and (S)-BEL at 23° C. for 3 min. Radiolabeled substrate (1-palmitoyl-2-[1-¹⁴C]-oleoyl-sn-glycero-3-phosphatidylcholine) dissolved in ethanol was then added to each reaction, mixed by vortexing, and incubated for 5 min at 37° C. Released [1-¹⁴C]-oleic acid was quantified as described more particularly hereafter.

FIG. 6A shows Recovered Triolein Lipase Activity of Sf9 Subcellular Fractions Containing Recombinant Human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10). Cytosol and membrane fractions were prepared from cells infected with either control pFastBac (pFB) baculovirus or baculovirus encoding human iPLA₂ε(His)₆(His₆ shown as SEQ ID NO: 10) and incubated in the presence of [9,10-³H(N)]-triolein at 37° C. for 15 min as described more particularly hereafter. Radiolabeled products and unreacted substrate were extracted into butanol, separated by thin layer chromatography, and released [9,10-³H]-oleic acid was quantified by scintillation spectrometry. Data presented are the averages (±S.E.) of three independent experiments performed in duplicate.

FIG. 6B shows Inhibition of Recombinant Human Adiponutrin (iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) Triolein Lipase Activity by BEL. Sf9 membranes from pFB control or human adiponutrin (iPLA₂ε(His)₆-expressing cells (iPLA₂ε) (His₆ shown as SEQ ID NO: 10) were incubated with 100 μM [9,10-³H(N)]-triolein in 85 mM potassium phosphate, pH 7.0 in the presence of 25 μM lecithin and 12.5 μM sodium taurocholate in the presence or absence of 10 μM BEL. Released [9,10-³H(N)]-oleic acid was extracted into butanol, resolved from remaining radiolabeled substrate and products by TLC, and quantified by scintillation spectrometry as described more particularly hereafter.

FIG. 6C shows Inhibition of Recombinant Human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) Triolein Lipase Activity by BEL. Affinity purified iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) was incubated with the indicated concentrations of BEL for 3 min at 23° C. Following addition of a buffered suspension of [9,10-³H(N)]-triolein, samples were incubated for 15 min at 37° C. as described more particularly hereafter. Radiolabeled products and unreacted substrate were extracted into butanol, separated by thin layer chromatography, and released [9,10-³H]-oleic acid was quantified by scintillation spectrometry. Data presented are the average values from four independent determinations.

FIG. 7 shows TALON-Co²⁺ Affinity Chromatography of Recovered Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10). The cytosolic fraction (20 ml) from Sf9 cells expressing recombinant human adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) was mixed by inversion with 2.5 ml of TALON-Co²⁺ affinity resin for 1 h at 4° C. The cytosol-resin suspension was poured into an empty Pharmacia column (1×10 cm) and washed with 8 column volumes of Buffer A (25 mM sodium phosphate, pH 7.8 containing 20% glycerol, 500 mM NaCl, and 2-mercaptoethanol). Bound human adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) was then eluted with a gradient of imidazole in Buffer A as indicated by the dashed line. Collected fractions were assayed for triolein lipase activity as described more particularly hereafter. The triolein lipase specific activity within peak fractions following elution of iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) from the Co²⁺-charged TALON column was 6.7±0.4 nmol of oleic acid·min⁻¹·mg protein⁻¹.

FIG. 8 shows Recombinant Human Adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) Catalyzes Transacylation of [¹⁴C]-Mono-olein (donor) to Mono-olein and Diolein (acceptors) to form Triolein. A. Sf9 cell cytosolic fractions from pFB control and human adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) (AdipoN) were incubated in 85 mM potassium phosphate buffer, pH 7.0 containing 2 mM EDTA, 1 mM DTT, 100 μM diolein (acyl acceptor), and 10 μM [oleoyl-1-¹⁴C]-mono-olein (acyl donor) at 37° C. for 30 min. Radiolabeled products and remaining substrate were extracted into butanol, resolved by TLC, and quantified by scintillation spectrometry as described more particularly hereafter.

FIG. 9 shows Affinity Purified Human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) Catalyzes Transacylation of Mono-olein to Form Diolein and Triolein. A, [¹⁴C-1]-diolein production from [¹⁴C-1]-mono-olein. B, [¹⁴C-1]triolein production from [¹⁴C-1]-mono-olein. Fractions from pFB control and human iPLA₂ε(His)₆(His₆ shown as SEQ ID NO: 10) were incubated with [¹⁴C-1]-mono-olein acyl donor in the presence or absence of 1,2-diolein (1,2-DOG) or 1,3-diolein (1,3-DOG) acyl acceptor at 37° C. for 15 min. Radiolabeled products and remaining substrate were extracted into butanol, resolved by TLC, and quantified by scintillation spectrometry as described more particularly hereafter. Data presented are the averages (±S.E.) of three independent experiments performed in duplicate.

FIG. 10 shows effective and successful Inhibition of 3T3L1 Triolein Lipase Activity by BEL. 3T3L1 adipocytes at Day zero, Day 4, and Day 8 of differentiation were harvested and lysed in 50 mM Tris-HCl, pH 7.0 containing 0.25 M sucrose, 1 mM EDTA, and 2 μg/ml leupeptin. Cell homogenates were assayed for total triolein lipase activity by incubating in 85 mM potassium phosphate, pH 7.0 containing 1 M NaCl, 25 μM lecithin, 12.5 μM sodium taurocholate, and 100 μM [9, 10-³H(N)]-triolein for 30 min at 37° C. Radiolabeled products ([9,10-³H(N)]-oleic acid) and remaining substrate were extracted into butanol, resolved by TLC, and quantified by scintillation spectrometry as described more particularly hereafter.

FIG. 11 shows our Modulation of Recombinant Human Adiponutrin (iPLA₂ε(His)6) (His₆ shown as SEQ ID NO: 10) Lipase/Transacylase Ratio by BEL Triolein lipase and transacylation (mono-olein (acyl-donor) to diolein (acyl-acceptor) to form triolein). Activities of recombinant human adiponutrin (iPLA₂ε. (His) 6) (His₆ shown as SEQ ID NO: 10) were measured in the presence and absence of 10 mM BEL as described in Test Procedures. Addition of BEL caused marked inhibition of iPLA₂ε(His)6) (His₆ shown as SEQ ID NO: 10) triolein lipase activity while having no effect on the transacylation activity of the enzyme.

FIG. 12 shows Quantitative PCR of iPLA₂ε Message in Mouse 3T3-L1 Preadipocytes and Human SW872 Liposarcoma Cells. Relative mouse iPLA₂ε (adiponutrin) mRNA levels (Panel A) in differentiating 3T3-L1 cells. Total RNA was extracted from 3T3-L1 cells on the day indicated, reverse transcribed, and the appropriate primer/probe sets were utilized to determine by quantitative PCR the relative amounts of mouse iPLA₂ε mRNA present as described more particularly hereafter. Data presented are representative of three independent experiments (average±S.E.). Panel B, quantitative PCR amplification curves for iPLA₂ε (solid circles) mRNA levels in SW872 cells. Total RNA was isolated from confluent SW872 cells, reverse transcribed, and the appropriate primer/probe sets were utilized to determine by quantitative PCR the relative amounts of human iPLA₂ε mRNA present as described more particularly hereafter. ΔRn indicates the change in relative fluorescence of the FAM reporter dye.

DETAILED DESCRIPTION OF THE INVENTION

The inventors have discovered (e.g. isolated and characterized) a human iPLA₂ε gene and variants and successful and isolated and recovered and characterized expressed proteins therefrom which is involved in the hydrolysis and recycling of the hydrolysis of lipids in fat cells of the human body. In connection therewith, the inventors identified and present for the first time the specific adipocyte human protein target iPLA₂ε. (See FIGS. 3A and 3B)

Further, the inventors have discovered a medical treatment for combating obesity and over-weightness in humans which comprises effectively administering an effective inhibiting amount of a compound which blocks or inhibits human iPLA₂ε expression or enzymatic activity in a living cell. In an aspect the living cell is in a human and a determination is made after such successful administration if the patient has changed weight. If so, it is determined that the treatment was successful.

The inventors have also discovered a useful screening method and research tool for identifying drugs which are useful to successfully hold weight in a living mammal or if desired to reduce weight gain.

In an aspect, this invention is used to identify an siRNA (and its staple chemical derivatives), antisense DNA or pharmaceutical compounds modulating the activity of iPLA₂ε which can then be injected, applied as salve, taken orally or otherwise placed in close spatial proximity of a targeted adipose depot where it can modulate the content of fat in said tissue or total weight, appetite or insulin sensitivity of a patient and thus in essence be used for body sculpting to provide a non surgical alternative to plastic surgery or other methods of fat removal and improved appearance.

In an aspect, this invention can be used through either antisense DNA, siRNA or pharmaceutical compounds to modulate the activity of iPLA₂ε and thereby alternate the release of endocrine regulators from fat cells thereby altering appetite, the leptin responsive genes, adiponectin release or those of other hormones released from the fat cell in response to the fat cell's loaded state which effect its endocrine function in a way to positively modify weight control, insulin sensitivity or physical appearance.

In an aspect, a suitable sequence for siRNA suitable for silencing a gene is obtained by providing Dharmacon, Inc. 1376 Miners Drive #101 Lafayette, Colo. 80026 with a suitable sequence of a gene to be silenced. Dharmacon employs a custom proprietary process to identify candidate siRNA based on the initial gene sequence from a submitter. In an aspect, siRNA is identified by providing Dharmacon with SEQ ID NO: 3.

The construction of a suitable vector can be achieved by any of the methods well-known in the art for the insertion of exogenous DNA into a vector. see Sambrook et al., 1989, Molecular Cloning, A Laboratory Manual, Cold Spring Harbor Press, N.Y.; Rosenberg et al., Science 242:1575-1578 (1988); Wolff et al., PNAS 86:9011-9014 (1989). For Systemic administration with cationic liposomes, and administration in situ with viral vectors, see Caplen et al., Nature Med., 1:39-46 (1995); Zhu et al., Science, 261:209-211 (1993); Berkner et al., Biotechniques, 6:616-629 (1988); Trapnell et al., Advanced Drug Delivery Rev., 12:185-199 (1993); Hodgson et al., BioTechnology 13:222 (1995).

In a further aspect, transfectamine is obtained from InVitrogen Corporation, 1600 Faraday Avenue, P.O. Box 6482, Carlsbad, Calif. 92008 and/or Calgene Inc., 1920 Fifth Street, Davis, Calif. 95616 and a mixture is prepared in a tissue culture. This tissue culture is taken in tumor cells which “eat” the admixture comprising siRNA. Without being bound by theory, it is believed that siRNA is an effective toxic agent against a gene comprising a polynucleotide having a sequence shown in SEQ ID NO: 3. Technical information which provides useful tools for identifying siRNA using a sequence of a polynucleotide such as SEQ ID NO: 3 can be found on the Whitehead Biocomputing group website. This information is incorporated herein in its entirety by reference.

In an aspect, the discovery and the sequences contained herein (protein, nucleic acid, SNPs and their covalent modifications in both complete sequence and salient parts) are used as biomarkers indicative of disease states related to lipid metabolism including but not limited to the metabolic syndrome, the diagnosing and worsening of obesity, and the efficacy of drug treatment for obesity, hypertension, atherosclerosis or inflammation. It is envisaged that cardiac risk, susceptibility to stroke, renal failure and/or diabetes will be more accurately assessed based upon the type, amount and modifications of the iPLA₂ε sequences described herein. Accordingly, its utility as both a biomarker for atherosclerosis, diabetes, incipient hypertension or heart attacks should be available from the judicious use of serum and biopsy samples (DNA sequencing for SNPs, post translational modifications, and amount and half live of salient entities) to develop effective pharmaceuticals (including but not limited to traditional low molecular weight entities, antisense DNA and siRNA) as well as to evaluate their efficacy in treatment or identifying specific subgroups who would most greatly benefit from such treatment.

As used herein, the term “compound” includes cell(s), compounds, ions/anions, cations and salts.

As used herein, the term “adipocyte” includes any cell storing fat.

As used herein, the term “siRNA” means functional short interfering RNA. Articles which describe the effects of small interfering RNA (siRNA) on silencing genes are 1. Elbashir, S M et al (2001) Nature, 411, 494-498; 2. Hannon, G J (2002) Nature, 418, 244-251 and 3. Tijsterman, M (2002) Annu. Rev. Genet., 36, 489-519, Instruction for siRNA construction is available from Silencer™ siRNA Construction Kit Instruction Manual, Catalog #: 1620, Ambion Inc., 2130 Woodward St., Austin, Tex. 78744-1832, USA. Instruction for siRNA transfection is available in Silencer™ siRNA Transfection Kit Instruction Manual, Catalog #: 1630, Ambion Inc., 2130 Woodward St., Austin, Tex. 78744-1832, USA. Additional information is available on Ambion's Technical Resources website at TechNotes Vol. 10:1.

The phrase “a sequence encoding a gene product” refers to a nucleic acid that contains sequence information, e.g., for a structural RNA such as rRNA, a tRNA, the primary amino acid sequence of a specific protein or peptide, a binding site for a transacting regulatory agent, an antisense RNA or a ribozyme. This phrase specifically encompasses degenerate codons (i.e., different codons which encode a single amino acid) of the native sequence or sequences which may be introduced to conform with codon preference in a specific host cell.

By “host cell” is meant a cell which contains an expression vector and supports the competent replication or expression of the expression vector. Host cells may be prokaryotic cells such as E. coli, or eukaryotic cells such as yeast, insect, amphibian, e.g. Xenopus, or mammalian cells such as HEK293, CHO, HeLa and the like.

As used herein, the term “administration” includes the effective administration which includes the application of a drug to a sample or to the body of a patient or research subject by injection, inhalation, ingestion, or any other effective means whereby the drug is presented to the target or area of intended delivery and reception of the drug. Normally after such administration the functional effects of the drug are detected as by suitable effective analytical means to determine the effect if any of the drug following its administration.

As used herein a “therapeutic amount” is an amount of a moiety such as a drug or compound which produces a desired or detectable therapeutic effect on or in a mammal administered with the moiety.

As used herein, an “expression vector” means a nucleic acid construct, generated recombinantly or synthetically, with a series of specific nucleic acid elements which permit competent transcription of a particular nucleic acid in a host cell. The expression vector can be part of a plasmid, virus, or nucleic acid fragment. Typically, the expression vector includes a nucleic acid to be transcribed operably linked to a promoter.

As used herein the term “putative” means deemed to be, supposed, reputed to be an inhibitor of the expression of iPLA₂ε in iPLA₂ε expressible tissue such as in adipose tissue of a transgenic mouse or a sample tissue thereof or a sample adequately representative thereof.

As used herein, the terms “compound” and “moiety” includes cell(s), compounds, ions/anions, cations and salts, including living cells of a life sustaining biosystem.

As used herein, the term “tissue” includes tissue, cells and collections of a multiplicity of homogenous or nearly homogenous cell lines or a sample thereof or an adequately representative sample thereof. In an aspect the tissue is a living mammalian tissue such as in a tissue culture or living mammal or in a living transgenic mouse.

As used herein, the term “peptide” is any of a group of compounds comprising two or more amino acids linked by chemical bonding between their respective carboxyl and amino groups. The term “peptide” includes peptides and proteins that are of sufficient length and composition to affect a biological response, e.g. antibody production or cytokine activity whether or not the peptide is a hapten. term “peptide” includes modified amino acids, such modifications including, but not limited to, phosphorylation, glycosylation, acylation prenylation, lipidization and methylation.

As used herein, the term “polypeptide” is any of a group of natural or synthetic polymers made up of amino acids chemically linked together such as peptides linked together. The term “polypeptide” includes peptide, translated nucleic acid and fragments thereof.

As used herein, the term “polynucleotide” includes nucleotide sequences and partial sequences, DNA, cDNA, RNA variant isoforms, splice variants, allelic variants and fragments thereof.

As used herein, the terms “protein”, “polypeptide” and “peptide” are used interchangeably herein when referring to a translated nucleic acid (e.g. a gene product). The term “polypeptide” includes proteins.

As used herein, the term “isolated polypeptide” includes a polypeptide essentially and substantially free from contaminating cellular components.

As used herein, the term “isolated protein” includes a protein that is essentially free from contamination cellular components normally associated with the protein in nature.

As used herein, the term “nucleic acid” refers to oligonucleotides or polynucleotides such as deoxyribonucleic acid (DNA) and ribonucleic acid (RNA) as well as analogs of either RNA or DNA, for example made from nucleotide analogs any of which are in single or double stranded form.

As used herein, the term “patient” and subject” are synonymous and are used interchangeably herein.

As used herein, the term “expression” includes the biosynthesis of a product as an expression product from a gene such as the transcription of a structural gene into mRNA and the translation of mRNA into at least one peptide or at least one polypeptide.

As used herein, the term “mammal” includes living animals including humans and non-human animals such as murine, porcine, canine and feline.

As used herein, the term “sample” means a viable sample of biological tissue or fluid and is not limited to heart tissue. Biological samples may include representative sections of tissues.

As used herein, the term “target protein” includes an amino acid sequence expressed on a target cell such as on a tumor cell. In an aspect, the target protein is a protein having a sequence shown in SEQ ID NO:1 or SEQ ID NO:2.

As used herein, the term “antisense” means a strand of RNA whose sequence of bases is complementary to messenger RNA.

As used herein, the term “siRNA” means short interfering RNA.

The phrase “a sequence encoding a gene product” refers to a nucleic acid that contains sequence information, e.g., for a structural RNA such as rRNA, a tRNA, the primary amino acid sequence of a specific protein or peptide, a binding site for a transacting regulatory agent, an antisense RNA or a ribozyme. This phrase specifically encompasses degenerate codons (i.e., different codons which encode a single amino acid) of the native sequence or sequences which may be introduced to conform with codon preference in a specific host cell.

By “host cell” is meant a cell which contains an expression vector and supports the replication or expression of the expression vector. Host cells may be prokaryotic cells such as E. coli, or eukaryotic cells such as yeast, insect, amphibian, e.g. Xenopus, or mammalian cells such as HEK293, CHO, HeLa and the like.

As used herein a “therapeutic amount” is an amount of a moiety such as a drug or compound which produces a desired or detectable therapeutic effect on or in a mammal administered with the moiety.

The term “recombinant” when used with reference to a cell, or protein, nucleic acid, or vector, includes reference to a cell, protein, or nucleic acid, or vector, that has been modified by the introduction of a heterologous nucleic acid, the alteration of a native nucleic acid to a form not native to that cell, or that the cell is derived from a cell so modified. Thus, for example, recombinant cells express genes and proteins that are not found within the native (non-recombinant) forms of the cell or express native genes that are otherwise abnormally expressed, under expressed or not expressed at all.

An “expression vector” includes a nucleic acid construct, generated recombinantly or synthetically, with a series of specific nucleic acid elements which permit transcription of a particular nucleic acid in a host cell. The expression vector can be part of a plasmid, virus, or nucleic acid fragment. Typically, the expression vector includes a nucleic acid to be transcribed and operably linked to a promoter so that it is functional.

Herein, the inventors identified isolated, purified and characterized a novel human iPLA₂, termed iPLA₂ε, which is homologous to mouse adiponutrin whose mRNA has been previously demonstrated to be strongly induced in vitro during differentiation of 3T3-L1 cells into adipocytes (1). Intriguingly mouse, adiponutrin mRNA rapidly increases when fasting mice are fed a high carbohydrate diet, rapidly decreases upon re-fasting, and is inappropriately upregulated in genetic models of obesity (1,2). However, here, for the first time, the inventors have identified and provide human adiponutrin as a triglyceride lipase/transferase and a transacylase and a phospholipase.

Herein, the inventors describe their cloning and heterologous expression of recovery of iPLA₂ε, in Sf9 insect cells and demonstrate that the enzyme iPLA₂ε possesses calcium-independent phospholipase A₂ activity selective for arachidonic acid and abundant amounts of triolein lipase activity as well as transacylase activity.

Furthermore, the inventors demonstrate herein that the phospholipase A₂ and triolein lipase activities of this enzyme are inhibited by (E)-6-(bromomethylene)-3-(1-naphthalenyl)-2H-tetrahydropyran-2-one (BEL), a mechanism-based suicide substrate inhibitor of all known iPLA₂ε. We represent that iPLA₂ε represents a valuable pharmacologic target whose successful modulation reduces the incidence of obesity and the clinical manifestations of type 2 metabolic syndrome. The metabolic syndrome (syndrome X) is diagnosed by 3 or more abnormal findings using five thresholds, triglyceride level, LDL cholesterol, fasting glucose, systolic blood pressure and waist size.

The inventors here for the first time identified, isolated, recovered, purified and characterized human iPLA₂ε and practical uses for human iPLA₂ε. In summary, the inventors identified the signature ATP consensus sequence (GXGXXG) and the active site seine nucleophile (GXSXG) (FIG. 2), in a human protein, termed iPLA₂ε which is homologous to mouse adiponutrin. In this application, the inventors describe the cloning and heterologous expression of human iPLA₂ε in Sf9 cells and demonstrate that the expressed recombinant enzyme possesses phospholipase A₂, triglyceride lipase and monoglyceride transferase activities which are inhibited by (E)-6-(bromomethylene)-3-(1-naphthalenyl)-2H-tetrahydropyran-2-one (BEL). Moreover, the inventors describe how human adiponutrin iPLA₂ε can catalyze anabolic fat synthesis by transesterification as shown in FIG. 1.

These results demonstrate that the affinity-purified iPLA₂ε can selectively hydrolyze polyunsaturated fatty acids at the sn-2 position which have previously been shown to be substrates for oxidative enzymes in signaling cascades. Accordingly, iPLA₂ε may serve to generate lipid 2^(nd) messengers of signal transduction.

Exemplary embodiments are described in the following examples. It is intended that the specification, together with the examples, be considered exemplary only.

EXAMPLES Test Procedures and Results

The inventors' successful cloning of Human Adiponutrin (iPLA₂ε)—PCR primers (5′-AAAGAATTCCACCATGTACGACGCAGAGCGCGG-CTGGAGCTT-3′ (SEQ ID NO: 13) and 5′-AAAAGTCGACTCAGTGATGGTGATGGTGATGCAG-ACTCTTCTCTAGTGAA-3′) (SEQ ID NO: 14) designed to introduce a C-terminal 6x His tag at the 3′ end of human adiponutrin coding sequence and to incorporate 5′-EcoRI and 3′-SalI restriction sites for subcloning into the baculoviral expression vector pFASTBac1. Full-length 1.4 kb human adiponutrin was amplified from ATCC IMAGE clone ID 4870514. After sequencing the insert and flanking sequences on both strands of the adiponutrin-pFASTBac1 construct to ensure the sequence integrity of the construct, a bacmid construct was prepared using the Bac-to-Bac Baculovirus Expression System protocol (Invitrogen) for subsequent Cellfectin-mediated transfection of Sf9 cells in 35 mm plates to produce infectious recombinant baculovirus. Amplified recombinant baculovirus was then used to infect a spinner culture of Sf9 cells for 72 h and the supernatant was collected as a high titer viral stock.

The inventors' successful expression of Human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) in Sf9 cells and Subcellular Fractionation—Sf9 cells at a density of approximately 1×10⁶ cells/ml were infected with either control baculovirus or recombinant baculovirus encoding human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) or at an multiplicity of infection of approximately 1. Forty-eight hours post-infection, cells were harvested by centrifugation (250×g for 10 min), washed once in ice-cold phosphate buffered saline, re-pelleted, and resuspended in lysis buffer (25 mM sodium phosphate, pH 7.8 containing 20% glycerol and 2 mM 2-mercaptoethanol). Cells were lysed by sonication (30×1 s bursts at 40% power) and centrifuged at 100,000×g for 1 h to separate cytosolic and membrane fractions. Cellular membranes were resuspended in a volume of lysis buffer equivalent to the volume of the cytosol fraction.

TALON-Co²⁺ Affinity Column Chromatography of our iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10)—The cytosolic fraction containing recombinant human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) was mixed by inversion with 10% volume of TALON-Co²⁺ resin for 1 h at 4° C. The resin-cytosol suspension was then poured into a column (1.5×10 cm) and washed with 4 column volumes of lysis buffer containing 500 mM NaCl (Buffer A). Recombinant iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) was eluted from the column utilizing a gradient of imidazole (250 mM) in Buffer A. Fractions were collected and assayed for phospholipase A₂ activity as described below.

Generation and Immunoaffinity successful Purification and recovery of Anti-Human iPLA₂ε Antibodies—A peptide corresponding to residues 295-310 of human iPLA₂ε (CRLEGDELLDHLRLSIL) (SEQ ID NO: 9) was coupled to maleimide-activated mariculture keyhole limpet hemocyanin according to the instructions of the manufacturer, emulsified with Freund's complete adjuvant, and injected subcutaneously into New Zealand white rabbits. At two week intervals, the rabbits were boosted with the peptide-KLH conjugate emulsified in Freund's incomplete adjuvant until seroconversion occurred. The iPLA₂ε peptide was coupled to activated thiol-Sepharose 4B for immunoaffinity purification of the anti-peptide antibodies. Immunoreactive rabbit antisera were diluted 1:10 with 10 mM Tris-HCl, pH 7.5, prior to application to the peptide affinity column equilibrated with the same buffer. The resin was extensively washed with 10 column volumes of 10 mM Tris-HCl, pH 7.5 containing 500 mM NaCl prior to elution of bound antibodies with 0.1 M glycine-HCl, pH 1.0, into collection tubes containing 1 M Tris-HCl, pH 9.0 (1:3 fraction volume). Antibodies were concentrated, dialyzed against phosphate-buffered saline containing 20% glycerol and stored at −80° C. prior to use.

Assay for Phospholipase A₂ Activity—Sample fractions were incubated in 100 mM Tris-HCl, pH 7.2 containing either 4 mM EGTA or 10 mM CaCl₂ (200 μl final volume) for 5-30 min at 37° C. in the presence of 1-palmitoyl-2-[1-¹⁴C]-oleoyl-sn-glycero-3-phosphatidylcholine, 1-palmitoyl-2-[1-¹⁴C]-1 mmoleoyl-sn-glycero-3-phosphocholine, or 1-palmitoyl-2-[1-¹⁴C]-arachidonyl-sn-glycerol-3-phosphocholine introduced by ethanolic injection. In some reactions, BEL at the indicated concentrations was added prior to the addition of radiolabeled substrate. Reactions were terminated by addition of 100 μl of butanol and extraction of the radiolabeled product and remaining substrate into the butanol layer by vigorous vortexing. Samples were spotted on LK6 Silica Gel 60 Å TLC plates, overlaid with oleic acid standard, dried, and developed in petroleum ether/ethyl ether/acetic acid (70:30:1). The region of the plate corresponding to the oleic acid standard (visualized by iodine staining) was scraped into scintillation vials and quantified by liquid scintillation spectrometry.

Assay for Triolein Lipase Activity—Sample fractions were incubated in 85 mM potassium phosphate, pH 7.0 containing 1 M NaCl (250 μl final volume) for 30 min at 37° C. in the presence of a suspension of 100 M [9,10-³H(N)]-triolein, 25 μM egg yolk lecithin, and 12.5 μM to 100 μM sodium taurocholate. In some reactions, BEL (10 μM final concentration) was added prior to the addition of radiolabeled substrate. After extraction of radiolabeled reaction product and remaining substrate into butanol, samples were spotted on TLC plates, overlaid with oleic acid standard, dried, and developed in chloroform/methanol/NH₄OH (65:25:5). The region of the plate corresponding to the oleic acid standard (visualized by iodine staining) was scraped into scintillation vials and quantified by liquid scintillation spectrometry.

Assay for Lipid Transacylase Activity—Highly purified Co²⁺-TALON affinity chromatographic fractions containing adiponutrin (iPLA₂ε (His) (His₆ shown as SEQ ID NO: 10) (50 μl) were incubated in 85 mM potassium phosphate, pH 7.0 (250 μl final volume) for 15-30 min at 37° C. in the presence of a suspension of 10 μM [1-¹⁴C]-mono-olein (acyl donor), 25 μM to 100 μM acyl-acceptor (mono-olein or diolein), 25 μM egg yolk lecithin, and 12.5 μM to 25 μM sodium taurocholate. In some reactions, BEL (10 μM final concentration) was added prior to the addition of radiolabeled substrate. After extraction of radiolabeled reaction product and remaining substrate into butanol, samples were spotted on TLC plates, overlaid with oleic acid standard, dried, and developed in petroleum ether/ethyl ether/acetic acid (70:30:1). The region of the plate corresponding to diolein or triolein standard (visualized by iodine staining) was scraped into scintillation vials and quantified by liquid scintillation spectrometry.

Quantitative PCR of iPLA₂ε Message in Differentiating 3T3-L1 Adipocytes and SW872 Human Liposacrcoma Cells. 3T3-L1 pre-adipocytes were cultured and differentiated as described previously (3). Human SW872 liposarcoma cells were cultured as described previously (4). 3T3-L1 cells at day 0 through day 6 of differentiation (2 day intervals) or SW872 cells were washed twice with ice-cold phosphate buffered saline and RNA was prepared following the RNeasy (Qiagen) protocol as described by the manufacturer. RNA (0.1-2 μg) was reverse transcribed using MultiScribe reverse transcriptase (TaqMan Gold RT-PCR kit, Applied Biosystems) by incubation for 10 min at 25° C. followed by 30 min at 48° C. and a final step of 5 min at 95° C. 20 ng of the resultant cDNA was used for each quantitative polymerase chain reaction. Primer/probe sets for quantitative PCR were designed using Primer Express software from PE Biosystems. Probes were 5′ labeled with reporter dye FAM (6-carboxylfluorescein), and 3′ labeled with quenching dye, TAMRA (6-carboxytetramethylrhodamine). Human iPLA₂ε forward (5′-GGCAAAATAGGCATCTCTCTT-ACC-3′) (SEQ ID NO: 15) and reverse (5′-GGAGGGATAAGGCCACTGTAGA-3′) (SEQ ID NO: 16) primers were paired with probe (5′-AACATACCAAGGCATCCACGACTTCGTC-3′) (SEQ ID NO: 17). Mouse iPLA₂ε forward (5′-ACTGCACGCGGTCACCTT-3′) (SEQ ID NO: 18) and reverse (5′-CACGAGGTCCATGAGGATCTC-3′) (SEQ ID NO: 19) primers were paired with probe (5′-TGTGCAGTCT-CCCTCTCGGCCGTATAAT-3′) (SEQ ID NO: 20). Quantitative PCR was carried out using TaqMan PCR reagents (Applied Biosystems) as recommended by the manufacturer with GAPDH primers and probe as an internal standard. Each PCR amplification was performed in triplicate for 2 min at 50° C., 10 min at 95° C., followed by 40 cycles of 15 s at 95° C. and 1 min at 60° C.

For SDS-PAGE, proteins were separated according to the method of Laemmli (5). For Western analyses, the separated proteins in SDS-PAGE gels were transferred to polyvinylidene difluoride membranes and subsequently probed with antibodies directed against the iPLA₂ε peptide in conjunction with a protein A-horseradish peroxidase conjugate. Protein concentrations were determined by the Coomassie Plus Protein Assay (Pierce) using BSA as standard.

To confirm our discovery that the observed sequence homology correctly identified a novel iPLA₂ gene, we cloned human adiponutrin (iPLA₂ε) (See FIGS. 3A and 3B) and heterologously expressed the C-terminal His₆-tagged protein in Sf9 cells. Expression of the human ortholog of adiponutrin in Sf9 cells resulted in the production of the anticipated 53 kDa protein that was predominantly present in the membrane-associated fraction as detected by Western analysis (FIG. 4). Measurement of phospholipase A₂ activity demonstrated that Sf9 cells expressing iPLA₂ε(His)₆ exhibited greater PLA₂ activity with 1-palmitoyl-2-[1-¹⁴C]-oleoyl-sn-glycero-3-phosphatidylcholine as substrate in comparison to wild type cells (FIG. 5A). Furthermore, human iPLA₂ε (His)₆, like other members of the iPLA₂ε family of enzymes, did not require calcium ion for activity (FIG. 5A). Following purification by TALON-Co²⁺ affinity chromatography, human iPLA₂ε(His)₆ was demonstrated to preferentially hydrolyze polyunsaturated acyl chains (linoleoyl and arachidonyl) at the sn-2 position of choline phospholipids (FIG. 5B). Inclusion of either enantiomer ((R) or (S)) of the mechanism-based suicide substrate BEL inhibited iPLA₂ε(His)₆ calcium-independent phospholipase activity with an IC₅₀ of approximately 1 μM (FIG. 5C).

Considering the ability of iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) to catalyze phosphatidylcholine hydrolysis and its specific expression in adipocytes (4), the inventors were interested to determine if iPLA₂ε could also catalyze the hydrolysis of triglycerides. Importantly, Sf9 cell cytosol and membranes containing recombinant human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10), reproducibly exhibited approximately 10-fold higher triolein lipase activity relative to control (pFB) cytosol and membrane fractions (FIG. 6A). Furthermore, the triglyceride lipase activity of iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) was completely inhibited by inclusion of 10 μM BEL (FIG. 6B). The IC₅₀ of the affinity purified human iPLA₂ε(His)₆ (His₆ shown as SEQ ID NO: 10) for inhibition of triglyceride lipase activity was determined to be≈0.1 μM (FIG. 6C). The expressed His-tagged adiponutrin bound to a metal chelating affinity column and triglyceride lipase activity and adiponutrin mass could be eluted with imidazole (FIG. 7).

To further substantiate the importance of adiponutrin (iPLA₂ε) in adipocyte lipid metabolism and cycling, the inventors demonstrated that recombinant human adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) could catalyze triolein (triglyceride) synthesis from mono-olein and/or diolein through a transacylation reaction or sequential transacylation. Incubation of Sf9 cell cytosol containing recombinant human adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) in the presence of [Oleoyl-1-¹⁴C]-mono-olein (acyl donor and acceptor) demonstrated synthesis of [¹⁴C]-triolein approximately 10-fold higher than that observed in control pFB reactions (FIG. 8). Following purification utilizing a TALON-Co²⁺ affinity column, recombinant human adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) was further demonstrated to catalyze [¹⁴C]-diolein (TAG Intermediate) synthesis from [Oleoyl-1-¹⁴C]-mono-olein (acyl donor and acceptor) (FIG. 9A) and [¹⁴C]-triolein triolein synthesis from [Oleoyl-1-¹⁴C]-mono-olien (acyl donor) and diolein (acyl acceptor) (FIG. 9B). Thus, the inventors discovered that human adiponutrin (iPLA₂ε(His)₆) (His₆ shown as SEQ ID NO: 10) is able to transfer acyl equivalents from mono-olein to either mono-olein or diolein acceptors resulting in net synthesis of diolein and triolein, respectively.

Upon differentiation, 3T3-L1 adipocytes (day 4 and day 8 after initiation of differentiation) express high levels of triglyceride lipase activity which is virtually at very, very low levels in undifferentiated cells (day 0). Since human adiponutrin (iPLA₂ε) possesses TAG lipase activity which is BEL-inhibitable, the inventors were interested to determine the ability of BEL to inhibit the TAG lipase activity present in differentiated 3T3-L1 adipocytes. As shown in FIG. 10, approximately 70% of the triolein lipase activity in homogenates of day 4 and day 8 3T3-L1 cells was inhibited by BEL, suggesting that adiponutrin (iPLA₂ε) or lipases similar to adiponutrin are expressed during differentiated 3T3-L1 cells into adipocytes.

Comparison of the sensitivity of the lipase and transacylase activities of recombinant highly purified human adiponutrin (iPLA_(2ε) (His)₆) (His₆ shown as SEQ ID NO: 10) to inhibition by BEL revealed that the triolein hydrolase activity of human adiponutrin is at least 10-fold more sensitive to BEL inhibition than is the transacylase activity (FIG. 11). Importantly, our discovery of this result demonstrates that the distinct catalytic activities (lipase and transacylase) of human adiponutrin can be independently modulated by a pharmacologic manipulation. To this end, pharmaceutical compounds which modulate the transacylase to lipase ratio of iPLA₂ε are an important pharmaceutical target.

To further examine the roles of iPLA₂ε in adipocyte biology, we determined iPLA₂ε mRNA levels of each isoform in both human SW872 liposarcoma cells and differentiating 3T3-L1 adipocytes. Previous Northern analyses have demonstrated the dramatic upregulation of adiponutrin (iPLA₂ε) mRNA during 3T3-L1 adipocyte differentiation (1). Quantitative PCR utilizing primers for mouse iPLA₂ε revealed a marked increase in message by day 6 (FIG. 12A). Human SW872 liposarcoma cells have been previously utilized in the study of lipoprotein receptor-mediated cholesterol homeostasis. Quantitative PCR utilizing primers for iPLA₂ε demonstrated high levels of expression for this iPLA₂ isoform in SW872 cells (FIG. 12B).

DISCUSSION

Mouse adiponutrin was first identified by others by differential hybridization as a mRNA species that was strongly induced during differentiation of 3T3 cells into adipocytes (1). Subsequent studies have shown mouse adiponutrin is an adipocyte specific protein whose mRNA is rapidly increased after feeding, vanishes quickly after fasting and is inappropriately upregulated in genetic models of obesity (1,2,6). It is also a downstream target of the thiazolidinediones (7).

In studies of hormone-sensitive lipase knockout mice, it has become apparent that other intracellular lipases exist in adipose since HSL K/O accumulated DAG identifying HSL as predominantly a DAG lipase activity (8). Evidence from multiple laboratories indicates that additional enzymes are important in adipocytes (9-11). However, the molecular identification of these other intracellular triglyceride lipases has thus far remained elusive until this discovery.

During fasting, fatty acids released from white adipose tissue undergo considerable re-esterification (recycling) into triglyceride pools (12). The fat cell specific expression of adiponutrin in conjunction with its temporarily coordinated responses to feeding and fasting in conjunction with the biochemical discovery presented herein make it likely that adiponutrin is the critical regulator of TAG hydrolysis and recycling by transacylation in the adipocyte.

In recent years fortunately a large number of combinatorial and other enhanced chemistry techniques have been developed which fortunately now allow large multimillion compound libraries of diverse compounds to be rapidly synthesized. Such techniques have the potential to greatly accelerate the discovery of compounds which have biologically useful therapeutic properties by providing large assemblies or collections of such diverse chemical compounds for biological screening. The capability to produce such large numbers of compounds for screening is a driver for new methods of screening which are not adversely affected by time and resource constraints. This produces a need for new screening methods and models to permit rapid screening of vast compound libraries.

The inventors' results unambiguously demonstrate that adiponutrin catalyzes the hydrolysis of lipids and this identifies the inventor's discovery of a method to screen for inhibitors of its enzymic activity thereby providing a new method and valuable research tool for identification of pharmaceutical agents that promote weight loss and/or decrease insulin requirements (i.e., increasing insulin sensitivity).

In this regard, (prophetic example) a transgenic animal model is prepared which is useful in such screening. In an aspect, the transgenic animal tissue model comprises a cellular entity having a vector providing a gene capably expressing human iPLA₂ε and the model is characterized as to at least one of weight, diet and serum fat analysis. The transgenic animal model representing a genetic model of obesity is fed a first predetermined diet and then a second predetermined diet comprising a compound selected from a library of available candidate compounds which are putative for weight reduction effect in a living mammal. After a predetermined interval of time and after consuming the diet comprising the compound, the animal model is weighed and a comparison is made between the weight of the animal model being maintained on the predetermined diet having the supplemental compound and the animal model being on a predetermined diet absent the compound. If the weight of the animal model is significantly lower for the model having received the diet containing the compound, then the determination is made that it is likely that the compound is a candidate weight reduction agent. The inference therefrom is that the compound functions as an inhibitor to the expression of iPLA₂ε, its adipocyte protein target, allowing that determination to be made.

A noninvasive method of using products of a gene comprising a polynucleotide having a sequence shown in SEQ ID NO:3 as an indicator of the effectiveness of administered candidate drug to a living mammal having competently integrated in its genome that gene, which comprises administering the candidate drug therapy to the mammal, obtaining a sample of the animal and analyzing the sample for the extent of presence of a iPLA₂ε, determining the extent that administration had on the mammal, thereby evaluating the effectiveness of the candidate drug, making a prioritization of the development of the drug based on that effectiveness. In an aspect prioritization includes ranking the drug as to its potential therapeutic capability as to treating obesity, reducing insulin dependence, increasing insulin sensitivity. In an aspect the mammal is a transgenic nonhuman mammal carrying the iPLA₂ε gene. Those of skill in the art will be aware of the known methods of competently integrating iPLA₂ε into the human genome.

In an aspect, a drug identified herein as an anti-obesity agent is effectively pharmacologically administered to a patient by any competent administrative means. In an aspect, a pharmacological effective amount would be delivered to the patient to provide or produce a desired lowering of fat content. In an aspect, an injection via a needle is employed to deliver an effective amount to a patient.

Following successful treatment, it may be desirable to have the patient undergo maintenance therapy to prevent the recurrence of the disease state, wherein the oligomer is administered in maintenance doses, ranging from 0.01 μg to 100 g per kg of body weight, once or more daily, to once every several years.

The specific mammalian dose is calculated according to the approximate body weight or body surface area of the patient or the volume of body space to be occupied. The dose will also be calculated dependent upon the particular route of administration selected. Further refinement of the calculations necessary to determine the appropriate dosage for treatment is routinely made by those of ordinary skill in the art. The amount of the composition actually administered will be determined by a practitioner, in the light of the relevant circumstances including the condition or conditions to be treated, the choice of composition to be administered, the age, weight, and response of the individual patient, the severity of the patient's symptoms, and the chosen route of administration.

The pharmaceutical compositions of the present invention may be effectively and successfully administered in a number of ways to mammals depending upon whether local or systemic treatment is desired and upon the area to be treated. Administration may be topical (including ophthalmic, vaginal, rectal, intranasal, transdermal), oral or parenteral. Parenteral administration includes intravenous drip, subcutaneous, intraperitoneal or intramuscular injection, or intrathecal or intraventricular administration.

Useful formulations for topical administration may include transdermal patches, ointments, lotions, creams, gels, drops, suppositories, sprays, liquids and powders. Conventional pharmaceutical carriers, aqueous, powder or oily bases, thickeners and the like may be necessary or desirable. Coated condoms, gloves and the like may also be useful.

Useful compositions for oral administration include powders or granules, suspensions or solutions in water or non-aqueous media, capsules, sachets or tablets. Thickeners, flavoring agents, diluents, emulsifiers, dispersing aids or binders may be desirable.

Useful compositions for intrathecal or intraventricular administration may include sterile aqueous solutions which may also contain buffers, diluents and other suitable additives.

Useful formulations for parenteral administration may include sterile aqueous solutions which may also contain buffers, diluents and other suitable additives.

In an aspect this type of screening may be done on a nontransgenic or normal (wild) type species of life.

In an aspect, the invention further comprises a method to measure and determine the metabolic effects if any on a living mammal by the effective administration of a drug to a patient wherein the effects are clinically detectable and determinable in the mammal's triglyceride cycling system utilizing an inhibitor of iPLA₂epsilon. In an aspect the invention comprises administering a drug to a living mammal to effect or modulate the triglyceride cycling system using an iPLA₂epsilon inhibitor. In an aspect the invention comprises delivering a compound to a mammal wherein the compound is delivered to the mammal to effect the futile cycle.

In an aspect, a method of TAG analysis and lipid analysis useful in this invention is carried out by using a method disclosed in U.S. patent application U.S. Ser. No. 10/606,601 filed Jun. 26, 2003, “Spectrometric Quantitation of Triglyceride Molecular Species”, Publication No. 2004-0063118, published Apr. 1, 2004 which is incorporated herein by reference in its entirety. A level of expression greater or less than expression in an absence of the substance selected to be measured indicates and is determinant of activity in modulating iPLA₂ε expression.

In a first embodiment, in regard to the method of analysis disclosed in U.S. Ser. No. 10/606,601 filed Jun. 26, 2003, the content of which are incorporated herein by reference, a method for the determination of TG individual (i.e. separate) molecular species in a composition of matter such as the above in a biological sample comprises subjecting the biological sample to lipid extraction to obtain a lipid extract and subjecting the lipid extract to electrospray ionization tandem mass spectrometry (ESI/MS/MS) providing TG molecular species composition as a useful output determination.

In an aspect, our inventive concept comprises analyzing a biological sample using electrospray ionization tandem mass spectrometry (ESI/MS/MS) and performing a two dimensional analysis with cross peak contour analysis on the output of the ESI/MS/MS to provide a fingerprint triglyceride individual (i.e. separate) molecular species.

Briefly, the inventive methods present a novel two-dimensional approach/method which quantitates individual molecular species of triglycerides by two dimensional electrospray ionization mass spectroscopy with neutral loss scanning. This method is also useful for polar lipid analysis by ESI/MS using conditions as outlined in U.S. Ser. No. 10/606,601 (see above filed Jun. 26, 2003, the contents of which are incorporated herein by reference) and is protected by a provisional patent and be reference herein. This method provides a facile way to fingerprint each patient's (or biologic samples) triglyceride composition of matter (individual molecular species content) and lipid composition of matter directly from chloroform extracts of biologic samples. Through selective ionization and subsequent deconvolution of 2D intercept density contours of the pseudomolecular parent ions and their neutral loss products, the individual molecular species of triglycerides and phospholipids can be determined directly from chloroform extracts of biological material. This 2D (two dimensional) approach comprises a novel enhanced successful functional therapy model for the automated determination and global fingerprinting of each patient's serum or cellular triglyceride and phospholipid profile content thus providing the facile determination of detailed aspects of lipid metabolism underlying disease states and their response to diet, exercise or drug therapy.

In an aspect of this inventive method, tandem mass spectroscopic separation of specific lipid class-reagent ion pairs is used in conjunction with contour density deconvolution of cross peaks resulting from neutral losses of aliphatic chains to determine the individual triglyceride molecular species from a biological sample (blood, liver, muscle, feces, urine, tissue biopsy, or rat myocardium).

In an aspect, a biological sample is processed in tandem mass spectrometer a first mass spectrometer set up in a tandem arrangement with another mass spectrometer. In that regard the biological sample can be considered as sorted and weighed in the first mass spectrometer, then broken into parts in an inter-mass spectrometer collision cell, and a part or parts of the biological sample are thereafter sorted and weighed in the second mass spectrometer thereby providing a mass spectrometric output readily and directly useable from the tandem mass spectrometer.

In an aspect, a pre-analysis separation comprises a separation of lipoproteins prior to lipid extraction. In an aspect, the pre-analysis separation comprises at least one operation or process which is useful to provide an enhanced biological sample to the electrospray ionization tandem mass spectrometry (ESI/MS/MS). In an aspect, a pre-analysis separation is performed on a biological sample and two compositions are prepared accordingly from the biological sample. In an aspect one composition comprises high density lipoproteins and another composition comprises low density lipoproteins and variants thereof comprised of intermediate densities which can, if necessary, be resolved by chromatographic or other density techniques.

Generally, a biological sample taken is representative of the subject from which or of which the sample is taken so that an analysis of the sample is representative of the subject. In an aspect a representative number of samples are taken and analyzed of a subject such that a recognized and accepted statistical analysis indicates that the analytic results are statistically valid. Typically the composition is aqueous based and contains proteinaceous matter along with triglycerides. For example, a human blood sample is sometimes used. Through use of this inventive method, a plasma sample can be analyzed and appropriate information from the plasma can be extracted in a few minutes. Alternatively, information can be taken from the cells in the blood as well.

In an aspect, serum is utilized as a biological sample. After whole blood is removed from a human body and the blood clots outside the body, blood cells and some of the proteins become solid leaving a residual liquid which is serum.

In an aspect a control sample is employed in the analysis.

In an aspect, the biological sample or a representative aliquot or portion thereof is subjected to lipid extraction to obtain a lipid extract suitable for ESI/MS/MS. In an aspect lipids are extracted from the sample which in an aspect contains a tissue matrix. Non-lipid contaminants should be removed from the lipid extract.

In one aspect lipid extraction is carried by the known lipid extraction process of Folch as well as by the known lipid extraction process of Bligh and Dyer. These useful lipid extraction process are described in Christie, W. W. Preparation of lipid extracts from tissues. In: Advances in Lipid Methodology—Two, pp. 195-213 (1993) (edited by W. W. Christie, Oily Press, Dundee) EXTRACTION OF LIPIDS FROM SAMPLES William W. Christie The Scottish Crop Research Institute, Invergowrie, Dundee DD2 5DA, Scotland all of which are incorporated herein in their entirety by reference. The useful Folch extraction process is incorporated herein in its entirety by reference (13).

Generally, lipid extraction is carried out very soon in time on the tissue matrix or immediately after removal (harvest) of tissues (tissue matrix) from humanely sacrificed organisms which have been living (carried out using and following acceptable animal welfare protocols). Alternatively, tissues are stored in such a way that they are conservatively preserved for future use. In an aspect, a lipid extract is provided and used to produce ionized atoms and molecules in the inventive analytical method as feed to the ESI mass spectrometer in our novel analysis method.

In an aspect a chloroform lipid extract is employed as a lipid extract composition fed to the ESI mass spectrometer. The effluent from the ESI is fed to the tandem mass spectrometer (i.e. from the exit of the ESI).

In an aspect, a Freezer Mill 6800 from Fisher Bioblock Scientific is used to finely pulverize soft or hard harvested tissues of a representative biological sample in one or two minutes in liquid nitrogen to render the tissue sufficiently pliable and porous for lipid extraction. Alternatively, the pulverization of the harvested tissue is carried out by subjecting the harvested tissue to hand directed mashing and pulverization using a hand directed stainless-steel mortar and pestle. In a further aspect, an enzymatic digestion is carried out on the harvested tissue which is harvested from a preserved cadaver.

In an aspect, lipids are contained in the lipid extract following the lipid extraction. Generally the extraction is a suitable liquid/liquid or liquid/solid extraction whereby the TGs are contained in the extract. In an aspect the extractant has sufficient solvating capability power and solvating capacity so as to solvate a substantial portion of the TG therein or substantially all of the TG present in the biological sample and is contained in the lipid extract.

In an aspect, chloroform is employed as an extractant to produce a useful lipid extract. Other useful extractants include but are not limited to those extractants which have a solvating power, capability and efficiency substantially that of chloroform with regard to the TG molecular species.

The inventive process creates charged forms of very high molecular weight TG molecules obtained via lipid extraction of a biological sample as a part of the process of detecting and analyzing biological samples containing TG.

In an aspect, in order to detect for and analyze ionized atoms and molecules such as TG molecular species in a biological sample, the lipid extract of that biological sample is used to produce ionized atoms and molecules by an ionization method such as electrospray ionization (ESI). As used herein, the term ESI includes both conventional and pneumatically-assisted electrospray mass spectrometry.

In use, the inventive procedure operates by producing droplets of a sample composition by pneumatic nebulization which compresses and forces a biological sample composition containing TG such as an analyte containing TG into a proximal end of a mechanical means housing or holding a fine sized orifice such as a needle or capillary exiting at the distal end of the orifice at which there is applied a sufficient potential. Generally the orifice is a very small bore full length orifice having an internal average diameter or bore in the range from about 0.2 to about 0.5 mm.

In an aspect, formation of a suitable spray is a critical operating parameter in ESI. Suitable solvent removable filters may be used to remove undesired solvents in the biological sample composition prior to being fed to the ESI. Generally high concentrations of electrolytes are avoided in samples fed to ESI.

The composition of materials of the means housing or holding the orifice and the orifice are compatible with the compositions of the biological sample to be processed through the orifice. Metallic and composition plastic compositions may be employed. In an aspect the orifice is a capillary or has a conical or capillary shape. In another aspect the orifice is cone shaped with the exterior converging from the proximate end to the distal end.

In an aspect, the biologic sample is forced through the orifice by application of air pressure to the sample at the proximate end of the orifice or the sample is forced through the orifice or capillary by the application of vacuum at the distal end of the orifice. The net result is that ions are suitably formed at atmospheric pressure and progress through the cone shaped orifice. In an aspect the orifice is a first vacuum stage and the ions undergo free jet expansion. A collector at the distal end of the orifice collects the ions and guides the ions to a tandem mass spectrometer (MS/MS).

REFERENCES

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While the discovery has been described in terms of various specific embodiments, those skilled in the art will recognize that the discovery can be practiced with modification within the spirit and scope of the discovery. 

1. A method for measuring activity of a calcium independent phospholipase A₂ε (iPLA₂ε) in a biological sample, the method comprising introducing into the biological sample a lipid substrate for cleavage of fatty acids by the iPLA₂ε, and measuring cleavage of the lipid substrate and/or quantifying the release of fatty acid from the lipid substrate.
 2. The method as set forth in claim 1, wherein the lipid substrate is a phospholipid substrate.
 3. The method as set forth in claim 2, wherein the iPLA₂ε cleaves fatty acid from the sn-2 position of the phospholipid substrate.
 4. The method as set forth in claim 2, wherein the iPLA₂ε has a sequence shown in SEQ ID NO: 1 or SEQ ID NO:
 2. 5. The method as set forth in claim 2, further comprising modulating the iPLA₂ε activity.
 6. The method as set forth in claim 5, wherein the method comprises increasing the iPLA₂ε activity.
 7. The method as set forth in claim 5, wherein the method comprises decreasing the iPLA₂ε activity.
 8. The method as set forth in claim 5, wherein the method comprises administering an iPLA₂ε inhibitor for modulating the iPLA₂ε activity.
 9. The method of claim 8, wherein the iPLA₂ε inhibitor is selected from the group consisting of a pharmacologic compound, an antisense DNA, an siRNA, and an antibody.
 10. The method as set forth in claim 9, wherein the pharmacologic compound is (E)-6-(bromoomethylene)-3-(1-naphthalenyl)-2H-tetrahydropyran-2-one (BEL).
 11. The method as set forth in claim 9, wherein the antibody binds to the sequence shown in SEQ ID NO:9.
 12. Modulating fatty acid utilization and cycling in a patient in need thereof using the method of claim
 5. 13. The method as set forth in claim 12, wherein the patient in need thereof is a human.
 14. The method as set forth in claim 13, wherein the patient in need thereof is selected from the group consisting of an obese patient and a diabetic patient.
 15. Treating a living mammal to increase insulin sensitivity and reduce insulin requirements using the method of claim
 5. 16. The method as set forth in claim 15, wherein the insulin requirement is reduced in whole or part.
 17. The method as set forth in claim 15, wherein the living mammal is a diabetic patient.
 18. A method of identifying substances which modulate iPLA₂ε activity, the method comprising contacting a candidate substance with cells capable of expressing iPLA₂ε, measuring the activity of iPLA₂ε using the method of claim 1, determining whether a level of activity greater or less than activity of iPLA₂ε in an absence of the substance indicates and whether it is determinant of activity in modulating iPLA₂ε expression and thereafter optionally determining that the substance modulated iPLA₂ε activity.
 19. A method as set forth in claim 18 wherein said iPLA₂ε has a sequence comprising SEQ ID NO: 1 or SEQ ID NO:
 2. 